Labeled Trimethylalkyl Ammonium Stearate

E.. Seeley M., Stewart. \Y. T.. J. Biol. Chem. 135. 189-95. (1940). (1 9 47). ... Carl. .4rch. Biochem. Biophjs. 31, 62-71. (1951). (6) Ikaiva. Mivosh...
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were added to give net final concentrations of 40 and 150 rng. per liter. I n the case of the blank, the solution was diluted with the proper amount of water. T h e aliquots of the resulting systems were then treated with 84% sulfuric acid in the manner described. At both levels the average percentage recovery amounted to approximately 96%.

Literature Cited (1) .4nderson. E.. Seeley M., Stewart. \Y. T.. J . Biol. Chem. 135. 189-95 (1940). (2) Berm:*+. E., J . .4gr. Rpsearch 75, 43-7 (1947). (3) Dischz. Z.: Biochem. Z . 189, 77-80 (1927). (4) Dreywood: R.: Ind. Eng. Chem..

.-lna/.Ed. 18, 191 (1946). (5) Ikawa. Miyoshi. Siemann. Carl. .4rch. Biochem. Biophjs. 31, 62-71 (1951). ( 6 ) Ikaiva. Mivoshi. Siemann. Carl? J . Bioi. Chem. 180, 923-31 (1949). R m i i e d f o r reriezr! O c t h r 9. 7957. .ic22. 1958. Con/rihutzon ‘Vo. 17d7, .\lassachusetts .-1grzcuiturni Ewjeriment Stntim, I *niwrsity qf .Ilassachusrtts. -Inihrrst. .\lass.

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A N I M A L GROWTH STIMULANITS

The Metabolic Fate of Carbon-141 Labeled Trimethylalkyl Ammonium Stearate

M. S. MAMEESH, H. E. SCHENDEL and B. CONNOR JOHNSON

-

Division of Animal Nutrition, University of Illinois, Urbana, 111.

Trimethylhexadecyl ammonium stearate labeled with carbon-1 4 in the one position of the hexadec:yl chain has been administered to rats orally, as a diet ingredient, and by injection intraperitoneally. This compound is highly insoluble in water and, therefore, appeared iunlikely to be absorbed from the intestinal tract or metabolized by the body, when given by injection. However, the compound was absorbed from the intestinal tract of both species ‘to a small extent, and the absorbed fraction was rapidly metabolized and excreted bly way of the gastrointestinal tract, urine, and respiratory carbon dioxide. Absorption of the compound appeared to be higher in the chick, but concentration of the label in the tissues was similar in both species.

M

which stimulate animal growth in controlled amounts, arv toxic in large doses. T o evaluate the biological effects of such compounds, feeding as well as metabolism experiments r u s t be conducted to demonstrate the growth-stimulating effect a t various levels of intake and to determine the ability of the animal to metabolize and excrete the compound, if it is absorbed, before it accumulates in the tissues to levels which could be toxic either to the animals involved or, indirectly, to man. I n these experiments, trimethylhexad e ~ y l - l - C ’ ~ - a m m o n i u mstearate, which has chick and swine growth-stimulating activity (7-3), was administered orally or by injection to rats and chicks and the distribution of the radioactivity in the tissues and excreta was determined. A N Y CHEMICAL COMPOUNDS,

Materials and Methods Experiments with Rats. I n experiment I (Table I), 5130 mg. of C14-labeled trimethylalkyl ammonium stearate [Arq u a d stearate (Dyiafac), Armour and Co.] was thoroughly mixed with each kilogram of a balanced synthetic diet. T h e diet contained sucrose, casein, and corn oil as sources of carbohydrate, protein, and fat, respectively. Two weanling male albino rats of the Sprague Dawley strain were fed on the above diet for periods of 22 and 25 days. T h e feces

and urine were collected over the whole period and the respiratory carbon dioxide for the last 48 hours. At the end of the feeding period, the rats were killed with ether, the livers and intestines were separated from the carcasses, and the intestinal contents were added to the feces. The radioactivity was measured by burning each sample with V a n Slyke combustion liquid and collecting the carbon dioxide in a n ionization chamber. The counts were made on a vibrating reed electrometer. I n experiment I1 (Tables I1 and 111), the labeled Arquad stearate was injected. Preliminary experiments showed that Arquad stearate was much more readily absorbed when given intraperitoneally than when administered subcutaneously. Two male albino rats weighing 124 and 126 grams were injected intraperitoneally with ? mg. of Arquad stearate suspended in 1.0 ml. of water. T h e rats were immediately placed in allglass metabolism cages for ? days. T h e respiratory carbon dioxide from rat I was collected in 12-hour fractions and the urine from rat I1 in 24-hour fractions. At the end of the seventh day, the rats were killed with ether, and the radioactivity was determined on the feces, urine, respiratory carbon dioxide, carcass, and liver. I n experiment I11 (Table IV), three male albino rats were fed CI4-labeled Arquad stearate a t the level of 500 mg.

per kg. of a synthetic diet for 7 days. The -4rquad stearate \vas then withheld from the diet. One rat was killed a t 0 hour. one after 48 hours, and one after 96 hours from withholding the compound ; their carcasses were assayed for radioactivity. Experiments with Chicks. T M O1day-old Columbian crossed with S e w Hampshire chicks were given a nutritionally adequate corn-soybean meal diet for 5 Meeks. At this point. 200 mg. of CI4-Arquad stearate were mixed with each kilogram of the diet. T h e chicks were placed in individual wire-bottomed cages in a ventilated hood. Food and water were provided ad lzbitum. T h e feces and urine of each chick were collected together for the first 4 days on the C14-Arquad stearate diet. O n the fifth day, both chicks were operated on to obtain a sample of urine uncontaminated with feces (4). This was accomplished on one chick. At the end of the seventh day on the C’4-Arquad stearate diet the chicks were sacrificed, feathered, a n d washed. T h e abdomen was split open by a midline incision and the liver and the gastrointestinal tract were removed, washed, and frozen. T h e radioactivity of the carcass and the organs examined was determined as before. Results and Discussion Table I shows the distribution of the

V O L . 6, NO. 8, A U G U S T 1 9 5 8

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Table 1. Fate of Orally Administered C14-Arquad Stearate (500 mg. per kg. diet) Rat I Rot// Initial wt.: g. 36.6 40.5 Final wt., g. 99.0 127.0 Experimental period, days 22 25 Feed intake, 8. 116.00 161.00 Arquad intake, mg. 58,OO 80.50 intake, w. 26.216 36.225 RECOVERY, % 94 33 93.97 4.27 3.37 0.33 0.28 0.09 0.06 0.07 0.02 0.75 0.9' 100.06 98.45

Feces Urine Carcass Liver Gut CO,. Total

~~~

Average

Table 111.

Excretion of C14-Arquad Stearate

Period,

Radioactivity,

Recovery,

Hours

PC.

%

CARBON DIOXIDE (Rat 0-12 0,0073 12-24 0,0040 24-36 0,0035 36-48 0 0040 48-60 0 0026 _ _ Total 0 0214

94.15 3.82 0.30 0.08 0.04 0.86 99.25

Table 11. Fate of Intraperitoneally Injected C14-Arquad Stearate

0-24 24-48 48-72 72-96 96-120 120-144 144-168 Total

I).. 0.230 0.126 0.110 0 126 0 082 ____ 0 674

URINE(Rat 1 1 ) ~ 0 7462 23 54 0 1891 5 96 0 1061 3 35 0 0610 1 92 0 0363 1 li 0 0301 0 9j 0 0403 1 21.2091 38.14 ~

a Specific activity of BaCOa too loiv to count from third day on. Fractionally collected every 12 hours during 7-day experiment. c Fractionally collected every 24 hours during 7-day experiment.

Table V. Fate of CI4-Arquad Stearate Orally Administered to Chicks (.i\pprox. 200 mg. Arquad per kg. of diet) Chick

I

Initial wt., g. 434 Final wt.. g. 51 1 Experimental period, days, 7 Feed intake, g. 259 .4rquad intake. mg. 51.8 C': intake, PC. 23.31 Carcass Ivt., mg. 345 Carcass Liver Gut Gizzard Crop Feces

%

contents 5.95 Total 66.54

Table IV. Residual Radioactivity in Carcasses of Rats Killed after C14-Arquad Stearate Was Withheld from Diet

Rat I Rat I/ Rat I Rof I f Feces 1.5400 1.5785 48.58 49.79 Urine 1,1140 1 2091 35.14 38.14 C O Y 0.0204 0.0581 0.64 1.83 Liver 0,0108 0 0219 0.34 0.69 Car0 48 96 cass 0.3836a 0.3789 12.104 11.95 Gut .. . 0.0243 , , , 0.77 Initial wt., g. 48 47 47 -~~~ Final wt., g. 76 83 94 Total 3.0688 3.2708 96.80 103.17 Feed intake, g. 51 43 49 a For Rat I this figure represents carcass Arquad intake, plus gut. mg. 25.5 21.5 24.5 pc. intake 11.475 9.675 11.025 Carcass wt. 67.3 69.85 78.55 yo recovery in carcassa 1.74 1.34 1.27 0 Intestinal contents were removed. radioactivity in the tissues and excreta of the rats following oral administration of C"-labeled .4rquad stearate. T h e apparent absorption of the compound was slight, 94% of the radioactivity being retestinal tract the urine, and the respiracovered in the feces (Table I). When labeled Arquad stearate was injected tory carbon dioxide; only 137, remained (Table 11). nearly one half of the inin the carcass tissues. Table 1L7 shoirs jected radioactivity was recovered in the that after withholding the labeled .4rquad stearate from the diet, the small feces during 7 days following the injecamount of radioactivity remaining in the tion. T h e true absorption of the orally administered .4rquad stearate was therecarcass was being slowlv excreted. T h e distribution of the activitv in the fore estimated to be about 10yo. Of this absorbed activity, 50% was extissues and excreta of the chick follo\ving creted by way of the gastrointestinal oral administration of labeled -4rquad tract, 387, by \ray of the urine, 8% by stearate (Table V) indicates that absorpway of the respiratory carbon dioxide, tion of the compound was greater in the and 47, remained in the carcass tissues. chick than in the rat. T h e uric acid Table I11 shobvs that excretion of the recovered from one chick did not label, by way of the respiratory carbon contain any measurable radioactivin . T h e unrecovered radioactivity, \L hich dioxide and the urine, was high during amounted to about 30% of the administhe first 24 hours following injection, tered dose, included losses in the respiradropped sharply the second day: then decreased gradually over the remaining 5 tor!' carbon dioxide. feathers. and represented the difficultv of quantitatively days of collection. Thus, during 7 days following injection of the labeled Arquad collecting chick excreta. These data show that in both species stearate, 87Yc of the injected radioactivity was excreted by way of the gastroinlittle of the compound is absorbed from

620

AGRICULTURAL

421 484

7

242 48.4 21.78 355

Recovery, Yo 7.44 4.31 0,73 0.46 2.06 1 .oo 0.40 0.57 0.15 0.18 49.81 53.66 ~

Recovery,

I/

Gut

(3.17pc.) pc. C ' 1

Chick

A N D F O O D CHEMISTRY

2 42 __

62.60

Specific activity of Carcass 2 3 X pc./g. tissue 3 9 X Liver X 10-3 pc./g. tissue 6 8 X 10-3 3 1 X pc. /ml. Bile The specific activity of the uric acid was too small to count.

the gastrointestinal tract and that which is absorbed can be metabolized both by oxidation to carbon dioxide and also by excretion both into the feces (presumably via the bile) and into the urine (b>conversion to a water-soluble compound). O n e dimensional paper chromatography of the rat urine followed by radioautography cf the developed chromatograms indicated the urinary excretion compounds to be different from the compound administered.

Acknowledgment This \york was supported in part by a grant-in-aid from .4rmour and Co., Chicago, 111. Literature Cited

(1) Balloun. S. L., Poultr! Sci. 34, 191 (1955). (2) Ely, C.M., Science 114, 523 (1951). (3) Luecke, R. I$'., Hoefer, J. A4., Thorp, F.. Jr., J . Animal Sci. 15, 765 (1956). (4) Sime. J. T . , Ph.D. thesis, p. 11. University of Illinois, Urbana, Ill., 1954. Receiaed f o r reziew December .iccepted iifiril 10, 1958.

23> 1957.